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使用FuGene将脂质介导的基因转移至原代神经元:与C6胶质瘤细胞和原代神经胶质细胞的比较

Lipid-mediated gene transfer into primary neurons using FuGene: comparison to C6 glioma cells and primary glia.

作者信息

Wiesenhofer B, Humpel C

机构信息

Laboratory of Psychiatry, University Hospital Innsbruck, Austria.

出版信息

Exp Neurol. 2000 Jul;164(1):38-44. doi: 10.1006/exnr.2000.7414.

Abstract

Gene transfer into cells of CNS origin is an important tool to counteract neurodegeneration by introducing, e.g., neuroprotective molecules. Although viral gene transfer reveals the highest gene transfer efficiency, liposome-mediated gene transfer seems to become an attractive alternative. In this study we investigated the lipid-mediated gene transfer into primary neurons in vitro by using the novel nonliposomal lipid FuGene and compared it to primary glia and malignant C6 glioma cells. FuGene-mediated gene transfer was useful to transfer the reporter gene beta-galactosidase into C6 glioma cells, primary glia, and primary neurons. Lipofection was highly dependent on the surface bottom and did not result in good efficiencies when using glass compared to plastic dishes. Comparing to a standard lipofection (1 x 8 h), lipofection on 3 consecutive days for 6 h each ("boosting") markedly increased the gene transfer efficiency in primary glia (up to sevenfold) and in primary neurons (up to sixfold). The use of endotoxin-free DNA only slightly increased the transfection efficiency. Immunohistochemistry demonstrated MAP-2-positive neurons (up to 1614 neurons/16-mm well; 2.4% of total neurons) as well as TH-positive neurons (up to 48 neurons/16-mm well; 12.7% of TH neurons) expressing beta-galactosidase. We conclude that FuGene-mediated gene transfer is an attractive alternative to introduce genes of interest into cells of glial and neuronal origin; however, this technique lacks sufficient gene transfer efficiency.

摘要

通过导入例如神经保护分子,将基因转移到中枢神经系统来源的细胞中是对抗神经退行性变的重要工具。尽管病毒介导的基因转移显示出最高的基因转移效率,但脂质体介导的基因转移似乎正成为一种有吸引力的替代方法。在本研究中,我们使用新型非脂质体脂质FuGene研究了脂质介导的基因在体外向原代神经元的转移,并将其与原代神经胶质细胞和恶性C6胶质瘤细胞进行了比较。FuGene介导的基因转移可有效地将报告基因β-半乳糖苷酶转移到C6胶质瘤细胞、原代神经胶质细胞和原代神经元中。脂质转染高度依赖于表面底部,与塑料培养皿相比,使用玻璃培养皿时效率不高。与标准脂质转染(1×8小时)相比,连续3天每天进行6小时的脂质转染(“增强”)显著提高了原代神经胶质细胞(高达7倍)和原代神经元(高达6倍)的基因转移效率。使用无内毒素的DNA仅略微提高了转染效率。免疫组织化学显示表达β-半乳糖苷酶的MAP-2阳性神经元(高达1614个神经元/16毫米孔;占总神经元的2.4%)以及TH阳性神经元(高达48个神经元/16毫米孔;占TH神经元的12.7%)。我们得出结论,FuGene介导的基因转移是将感兴趣的基因导入神经胶质细胞和神经元来源细胞的一种有吸引力的替代方法;然而,该技术缺乏足够的基因转移效率。

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